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Fml1 的 ATP 酶活性对于其在同源重组和 DNA 修复中的作用至关重要。

The ATPase activity of Fml1 is essential for its roles in homologous recombination and DNA repair.

机构信息

Department of Biochemistry, University of Oxford, Oxford OX1 3QU, UK.

出版信息

Nucleic Acids Res. 2012 Oct;40(19):9584-95. doi: 10.1093/nar/gks715. Epub 2012 Jul 27.

Abstract

In fission yeast, the DNA helicase Fml1, which is an orthologue of human FANCM, is a key component of the machinery that drives and governs homologous recombination (HR). During the repair of DNA double-strand breaks by HR, it limits the occurrence of potentially deleterious crossover recombinants, whereas at stalled replication forks, it promotes HR to aid their recovery. Here, we have mutated conserved residues in Fml1's Walker A (K99R) and Walker B (D196N) motifs to determine whether its activities are dependent on its ability to hydrolyse ATP. Both Fml1(K99R) and Fml1(D196N) are proficient for DNA binding but totally deficient in DNA unwinding and ATP hydrolysis. In vivo both mutants exhibit a similar reduction in recombination at blocked replication forks as a fml1Δ mutant indicating that Fml1's motor activity, fuelled by ATP hydrolysis, is essential for its pro-recombinogenic role. Intriguingly, both fml1(K99R) and fml1(D196N) mutants exhibit greater sensitivity to genotoxins and higher levels of crossing over during DSB repair than a fml1Δ strain. These data suggest that without its motor activity, the binding of Fml1 to its DNA substrate can impede alternative mechanisms of repair and crossover avoidance.

摘要

在裂殖酵母中,DNA 解旋酶 Fml1 是同源重组(HR)驱动和调控机制的关键组成部分,它是人类 FANCM 的同源物。在 HR 修复 DNA 双链断裂时,它限制了潜在有害交叉重组体的发生,而在停滞的复制叉处,它促进 HR 以帮助它们恢复。在这里,我们突变了 Fml1 的 Walker A(K99R)和 Walker B(D196N)基序中的保守残基,以确定其活性是否依赖于其水解 ATP 的能力。Fml1(K99R)和 Fml1(D196N)都能有效地结合 DNA,但完全不能解开 DNA 并水解 ATP。体内实验表明,这两种突变体在受阻复制叉处的重组减少程度与 fml1Δ 突变体相似,这表明 Fml1 的水解 ATP 驱动的马达活性对其促进重组的作用至关重要。有趣的是,与 fml1Δ 菌株相比,fml1(K99R)和 fml1(D196N)突变体在遭受遗传毒性时更为敏感,并且在 DSB 修复过程中发生更多的交叉。这些数据表明,没有其马达活性,Fml1 与 DNA 底物的结合可能会阻碍替代修复机制和避免交叉。

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